EP2271207A2 - Insertion efficace d adn dans des cellules souches embryonnaires - Google Patents

Insertion efficace d adn dans des cellules souches embryonnaires

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Publication number
EP2271207A2
EP2271207A2 EP09723802A EP09723802A EP2271207A2 EP 2271207 A2 EP2271207 A2 EP 2271207A2 EP 09723802 A EP09723802 A EP 09723802A EP 09723802 A EP09723802 A EP 09723802A EP 2271207 A2 EP2271207 A2 EP 2271207A2
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European Patent Office
Prior art keywords
type
site
sites
gene sequence
sequence
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EP09723802A
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German (de)
English (en)
Inventor
Jost Seibler
Nico Scheer
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ITI Scotland Ltd
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ITI Scotland Ltd
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Priority claimed from GB0805487A external-priority patent/GB0805487D0/en
Priority claimed from GB0903120A external-priority patent/GB0903120D0/en
Application filed by ITI Scotland Ltd filed Critical ITI Scotland Ltd
Publication of EP2271207A2 publication Critical patent/EP2271207A2/fr
Withdrawn legal-status Critical Current

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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K49/00Preparations for testing in vivo
    • A61K49/0004Screening or testing of compounds for diagnosis of disorders, assessment of conditions, e.g. renal clearance, gastric emptying, testing for diabetes, allergy, rheuma, pancreas functions
    • A61K49/0008Screening agents using (non-human) animal models or transgenic animal models or chimeric hosts, e.g. Alzheimer disease animal model, transgenic model for heart failure
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K67/00Rearing or breeding animals, not otherwise provided for; New or modified breeds of animals
    • A01K67/027New or modified breeds of vertebrates
    • A01K67/0275Genetically modified vertebrates, e.g. transgenic
    • A01K67/0278Knock-in vertebrates, e.g. humanised vertebrates
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    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/63Introduction of foreign genetic material using vectors; Vectors; Use of hosts therefor; Regulation of expression
    • C12N15/79Vectors or expression systems specially adapted for eukaryotic hosts
    • C12N15/85Vectors or expression systems specially adapted for eukaryotic hosts for animal cells
    • C12N15/86Viral vectors
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
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    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/87Introduction of foreign genetic material using processes not otherwise provided for, e.g. co-transformation
    • C12N15/90Stable introduction of foreign DNA into chromosome
    • C12N15/902Stable introduction of foreign DNA into chromosome using homologous recombination
    • C12N15/907Stable introduction of foreign DNA into chromosome using homologous recombination in mammalian cells
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
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    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/0004Oxidoreductases (1.)
    • C12N9/0071Oxidoreductases (1.) acting on paired donors with incorporation of molecular oxygen (1.14)
    • C12N9/0077Oxidoreductases (1.) acting on paired donors with incorporation of molecular oxygen (1.14) with a reduced iron-sulfur protein as one donor (1.14.15)
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2207/00Modified animals
    • A01K2207/15Humanized animals
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2217/00Genetically modified animals
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2217/00Genetically modified animals
    • A01K2217/07Animals genetically altered by homologous recombination
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2217/00Genetically modified animals
    • A01K2217/07Animals genetically altered by homologous recombination
    • A01K2217/072Animals genetically altered by homologous recombination maintaining or altering function, i.e. knock in
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2217/00Genetically modified animals
    • A01K2217/15Animals comprising multiple alterations of the genome, by transgenesis or homologous recombination, e.g. obtained by cross-breeding
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2217/00Genetically modified animals
    • A01K2217/20Animal model comprising regulated expression system
    • A01K2217/206Animal model comprising tissue-specific expression system, e.g. tissue specific expression of transgene, of Cre recombinase
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2227/00Animals characterised by species
    • A01K2227/10Mammal
    • A01K2227/105Murine
    • CCHEMISTRY; METALLURGY
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    • C12N2710/00MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA dsDNA viruses
    • C12N2710/00011Details
    • C12N2710/14011Baculoviridae
    • C12N2710/14111Nucleopolyhedrovirus, e.g. autographa californica nucleopolyhedrovirus
    • C12N2710/14141Use of virus, viral particle or viral elements as a vector
    • C12N2710/14143Use of virus, viral particle or viral elements as a vector viral genome or elements thereof as genetic vector

Definitions

  • the present invention relates, in general, to a method for introducing a heterologous replacement gene sequence into a host embryonic stem cell to replace an endogenous host gene target sequence.
  • the invention relates to a method for inserting large pieces of DNA into embryonic stem cells with improved efficiency, by first deleting the endogenous host gene target sequence, and subsequently utilising two proximally positioned site-specific recombinase target (RT) sites to insert a heterologous replacement gene sequence into the host chromosome.
  • RT site-specific recombinase target
  • mice have been produced through pronuclear injection of exogenous DNA.
  • mice have been generated by fusing an embryonic stem cell with a cell containing a Bacterial Artificial Chromosome (BAC) or a Yeast Artificial Chromosome (YAC) comprising the exogenous gene of interest and a selectable marker to assess integration of the exogenous DNA segment into the embryonic cell genome, as described in WO94/02602, for example.
  • BAC Bacterial Artificial Chromosome
  • YAC Yeast Artificial Chromosome
  • Such methods rely on integration of the BAC or YAC into the embryonic stem cell genome through the process of homologous recombination. Due to the technical demands involved in handling BACs and YACs, and the low transfection rates of ES cells when using large DNA constructs, transgenesis in this manner is time- consuming, inefficient and inaccurate.
  • US2007/0061900 describes a method for the humanisation of the heavy and light chain immunoglobulin variable region gene loci. This method involves the insertion into each of two vectors, termed LTVECs, of a site-specific recombination site arranged so as to be contiguous to a portion of the human immunoglobulin variable region. These LTVECs are then linearised and introduced into the genome of a mouse cell by homologous recombination, so that the site-specific recombination sites flank the mouse immunoglobulin variable region sequences, and the partial human immunoglobulin variable region sequences flank the site-specific recombination sites.
  • LTVECs two vectors
  • Effecting site-specific recombination excises the mouse immunoglobulin variable region sequence and joins the two partial human immunoglobulin variable region sequences, with the residual site-specific recombination site contained within it.
  • the resulting mice produce hybrid antibodies containing human variable and mouse constant regions, with subsequent transformation steps required to allow production of pure human antibodies.
  • this approach is inefficient, due to the low frequency of homologous recombination with vectors that carry very large sequences of heterologous DNA.
  • the segmental nature of the immunoglobulin variable region allows the residual site-specific recombination site to remain within the nucleic acid sequence with little chance of a detrimental effect.
  • RMGR recombinase-mediated genomic replacement
  • this method is inefficient for the insertion of large pieces of DNA due to the considerable distance between the non-interacting site-specific recombination sites present on the mouse chromosome and in the BAC. This distance is inevitable due to the presence of the mouse allele in the mouse chromosome at the time of recombination, and the reciprocal nature of the recombinatorial exchange.
  • the invention sets out to provide more generally applicable methods for selecting correctly targeted clones. Provision of an improved general method of selecting such clones will allow recombinatorial exchange to be performed in cells other than an HPRT-deficient (hprt " ) embryonic stem cell line. A universal selection method would also allow such a procedure to be conducted in any embryonic stem cell.
  • a method of introducing a heterologous replacement gene sequence into a host cell to replace an endogenous host gene target sequence comprising: a) incorporating a pair of identical site-specific recombinase target (RT) sites of type I into the same allele of a host chromosome in separate homologous recombination steps such that the endogenous host gene target sequence that is to be replaced is flanked on each side by said identical type I RT sites; wherein one of the identical type I RT sites is flanked by a type II RT site positioned proximal to the type I RT site, wherein the type II RT site is different to the type I RT site such that it is heterospecific, and as such cannot interact with the type I RT site and; b) effecting recombination between said pair of type I site-specific recombination sites such that the endogenous host gene target sequence is excised, and whereby a residual type I RT site remains in the
  • FIG. 1 A simple schematic of the mechanism of the invention is shown in Figure 1.
  • two type 1 RT sites are incorporated into the endogenous host cell chromosome of a host cell by two separate conventional homologous recombination reactions.
  • Homologous recombination is a phenomenon well known in the art, yet for ease of comprehension, a schematic of the mechanism of homologous recombination is shown in Figure 2.
  • the two recombination reactions are facilitated by short regions of homology between the endogenous host cell chromosome and the replacement nucleic acid sequence that comprises the type I RT site. These regions of homology facilitate strand invasion and subsequent base pairing, allowing strand elongation which inserts each recombination site into the host cell chromosome.
  • a type II RT site is also incorporated into the endogenous host cell chromosome, proximal to, and flanking the type I RT site.
  • the insertion of the two type I RT sites and one type II RT site into the endogenous host cell chromosome results in the arrangement shown in Figure 1.
  • the type I RT sites should thus flank the endogenous host gene target sequence, with one of the type I RT sites additionally flanked by a type II RT site, such that the type I RT site is positioned between the type II RT site and the endogenous host gene target sequence. Both type I RT sites should be aligned in the same direction, as shown in Figure 1 , so as to allow their recombination together in due course. It is known in the art that site-specific recombinases can be utilised to target homologous recombination to specific chromosomal locations (see Jessen et ah, 1997).
  • site specific recombinases allow recombination to be initiated upon demand by the addition of the site-specific recombinase.
  • site-specific recombination can then be effected between the two type I RT sites in the host cell.
  • Figure 3 the mechanism of site specific recombination is illustrated in Figure 3. These recombination events result in excision of the endogenous host gene target sequence, leaving the residual type I RT site positioned proximal to the type II RT site within the host cell chromosome.
  • This intermediate stage represents the production of a host cell in which the endogenous gene is knock-out (a knock-out ES cell).
  • the next stage in the methodology is to provide a heterologous replacement gene sequence.
  • the heterologous replacement gene sequence is located between a flanking type I RT site and a flanking type II RT site.
  • the RT sites are aligned in the same direction as the corresponding RT sites in the host cell chromosome, so as to allow their recombination together in due course.
  • the heterologous replacement gene sequence may be located within a vector, or may be a linear nucleic acid sequence.
  • the heterologous replacement gene sequence is located within a vector.
  • the method of the invention has a number of advantages. Firstly, the use of site-specific recombination for the insertion of the heterologous replacement gene sequence into the host cell chromosome allows for greatly improved efficiency over homologous recombination.
  • the method described in US2007/0061900 utilises homologous recombination for the insertion of a portion of the human immunoglobulin variable region which is contained within a linearised LTVEC.
  • the large size of the replacement sequence necessitates long DNA homology arms to facilitate homologous recombination between the host cell chromosome and the heterologous replacement gene sequence, which leads to corresponding inefficiencies.
  • the method of the present invention utilises site-specific recombination, which does not require long DNA homology arms to effect recombination, and the efficiency is therefore greatly improved.
  • the use of site-specific recombination for the insertion of the heterologous replacement gene sequence negates the need for large size homology arms, and allows the verification of correctly targeted cell clones by Southern blot analysis.
  • the mechanism of site-specific recombination is used for the insertion of the heterologous DNA sequence, as in the present invention, a greatly improved efficiency is evident.
  • the method of the present invention allows the complete replacement of an endogenous host gene target sequence with a heterologous replacement gene sequence in just a few rounds of targeting in host cells.
  • excision of the endogenous host gene target sequence generates a knockout cell, which acts as an intermediate in the method.
  • This can be usefully exploited, separately from the ultimate goal of successful introduction of the heterologous gene sequence, and allow analysis of the function of the excised endogenous host gene target sequence by looking at the effect of its deletion.
  • the ultimate insertion of the heterologous replacement gene sequence can allow comparison of the function of the replacement gene sequence with that of the endogenous gene sequence and the complete knock-out.
  • a further advantage of the present invention concerns the proximal positioning of the type I and type II RT sites in the host cell chromosome after excision of the endogenous gene sequence.
  • the frequency of correct targeting in a host chromosome where the RT sites are separated on different entities is less than 1x10 " .
  • the residual type I RT sequence and the type II RT sequence are positioned proximally
  • a "proximal" position resides within 100 nucleotides, preferably within 50 nucleotides, more preferably, within 40, 30, 20, 15, 10, 5 or less of another..
  • This positioning greatly increases the efficiency of insertion of the heterologous replacement gene sequence, and has lead to a targeting efficiency with the method of the present invention which can be as high as 1x10 " ⁇ .
  • This is an important benefit as obtaining correctly targeted embryonic stem cells is generally the rate limiting step in the generation of embryonic stem cells with a replacement of an endogenous host gene target sequence with a heterologous replacement gene sequence.
  • the lengths of DNA used by Wallace are so long (of the order of 200kb), there is a much increased opportunity for intramolecular rearrangements and undesired homologous recombination events to occur, which increases the chance of a non-functional or incorrect DNA structure being created.
  • the method of the present invention is advantageous in view of the Wallace method because the greatly increased efficiency allows the skilled person to start with many more clones in order to identify those in which the integrity and fidelity of the heterologous sequence is maintained.
  • the introduced heterologous replacement gene sequence may be incorporated under the control of its own regulatory sequences.
  • the genetic recombination events can be arranged so that the equivalent host cell regulatory sequences are situated upstream of the inserted heterologous replacement gene sequence and thus used in their place.
  • it will be desired to retain the host cell regulatory sequences rather than incorporate the regulatory sequences that are thought to govern transcription of the heterologous replacement gene sequence.
  • the regulatory sequences associated with the heterologous replacement gene sequence may be unable to control expression of the heterologous replacement gene sequence in the host cell.
  • One advantage of the methodology of the invention over conventional techniques, where integration of a heterologous replacement gene sequence into a host cell chromosome is more or less random, is that integration at the site of the equivalent host cell gene sequence ensures that the genomic context of gene placement is retained. By integrating at such a site, it is likely that the local chromosome structure is "open" in the sense that access to the chromosomal DNA is possible for transcription factors and other proteins required for transcription to take place. Not only this, but the same chromosomal context is retained as for the endogenous host gene sequence, such that regulation of DNA transcription at the level of the tertiary structure of the chromosome, by way of histone binding, and local folding/unfolding of the chromosome, is retained.
  • FIG. 1 Schematic of the methodology of the invention.
  • the method provides a mechanism of introducing a heterologous replacement gene sequence into a host embryonic stem cell to replace an endogenous host gene target sequence, comprising the insertion of two type I RT sites to flank the endogenous host gene target sequence, one of which is flanked by a type II RT sequence, effecting site-specific recombination between the type I RT sites to excise the endogenous host gene target sequence, providing a vector comprising a heterologous replacement gene sequence flanked by a type I RT site and a type II RT site, and effecting recombination between the corresponding RT sites present on the host cell chromosome and on the vector such that the heterologous gene sequence is introduced at the position in the host chromosome previously occupied by the host target gene.
  • FIG. 1 Mechanism of homologous recombination. Homologous recombination occurs following a double stranded chromosomal break. 5' to 3' exonuclease activity produces a 3' overhang and allows strand invasion to occur. DNA synthesis utilises the intact strand as a template and ligation repairs the chromosomal break generating a Holliday junction. Subsequent branch migration and resolution produce recombinant products.
  • FIG. 1 A) The LoxP site-specific recombination site.
  • FIG. 4 Method for the production of a transgenic mouse.
  • a transgenic mouse is produced by the insertion of one or more altered embryonic stem cells into a developing blastocyst. The blastocyst is then implanted into a pseudo-pregnant mouse and allowed to develop, producing a chimera.
  • Figure 5. Strategy for the deletion of the mouse Cyp3a cluster.
  • A Schematic representation of the chromosomal organisation and orientation of functional genes within the mouse Cyp3a Cluster (adapted from Nelson et al, 2004). Pseudogenes are not listed.
  • B Exon/Intron structure of Cyp3a57 and Cyp3a59. Exons are represented as black bars and the ATGs mark the translational start sites of both genes.
  • Cyp3a57 left and Cyp3a59 (right) by homologous recombination.
  • LoxP , Iox5171,frt and/? sites are represented as white, striped, black or grey triangles, respectively.
  • D Genomic organisation of the Cyp3a Cluster in double targeted ES cells after homologous recombination on the same allele at the Cyp3a57 and Cyp3a59 locus.
  • TK Thymidine Kinase expression cassette
  • Hygro Hygromycine expression cassette
  • ZsGreen ZsGreen expression cassette
  • P Promoter that drives the expression of Neomycin
  • 5' ⁇ Neo ATG-deficient Neomycin.
  • Figure 6 Strategy for the humanisation of the mouse Cyp3a Cluster.
  • A Initial configuration after Cre-mediated deletion of the Cyp3a Cluster as already depicted in Figure 5E.
  • B Modified human BAC comprising the human CYP3A4 and CYP3A7 genes used for Cre-mediated insertion into the deleted mouse Cyp3a Cluster.
  • C Genomic organisation of the Cyp3a Cluster in correctly targeted ES cells after Cre- mediated insertion of the human BAC.
  • D Deletion of the hygromycin and neomycin selection cassettes after F/p-mediated recombination at the frt and f3 sites. For the sake of clarity sequences are not drawn to scale.
  • Hygro Hygromycine expression cassette
  • P Promoter that drives the expression of Neomycin
  • 5' ⁇ Neo ATG-deficient Neomycin.
  • Figure 7. PCR analysis of 3 G418 resistant clones
  • A Genomic organisation of the Cyp3a gene cluster in correctly targeted ES cells after Cre-mediated insertion of the human BAC, as depicted in Figure 6C.
  • PCR primers used for PCR analysis are shown as black arrows, and expected PCR fragments are show as grey boxes.
  • B PCR results showing that all 3 clones carry a correct insertion of the human BAC.
  • FIG. 8 Southern analysis of 3 G418 resistant clones
  • A Genomic organisation of the Cyp3a gene cluster in correctly targeted ES cells after Cre-mediated insertion of the human BAC, as depicted in Figure 6C. The Southern probe used for Southern blot analysis is shown as a black line, and the expected restriction fragments are indicated.
  • B Southern blot results showing that all clones carry a correct insertion of the human BAC, and that clone 3 has an additional insertion.
  • FIG. 9 Hepatic CYP3A4 protein in humanised CYP3A4 mouse lines Southern blot results showing the presence of human CYP3 A4 in the liver of Cyp3a knockout mice.
  • FIG. 10 Intestinal CYP3A4 protein in humanised CYP3A4 mouse lines Southern blot results showing the presence of human CYP3A4 in the intestine of Cyp3a knockout mice.
  • CYP3A7 is the major CYP3A isoform expressed in human fetal liver, undergoes a developmental switch in the first week of postnatal life, with CYP3A7 virtually disappearing concomitant with transcriptional activation of the CYP3 A4 gene. A similar developmental switch has also been observed in the mouse (Cyp3al6 to Cyp3al l). The mouse used our experiment was over 9 weeks old and therefore, the expression of CYP3A7 might be switched to CYP3A4.
  • Figure 13 Hepatic CYP3A4 and Cyp3a protein expression in humanised CYP3A4 mouse lines Southern blot results showing the presence of human CYP3 A4 in the liver of Cyp3a knockout mice.
  • FIG. 14 Intestinal CYP3A4 and Cyp3a protein expression in humanised CYP3A4 mouse lines Southern blot results showing the presence of human CYP3A4 in the intestine of Cyp3a knockout mice.
  • CYP3A4 is catalytically active in CYP3A4/3A7_Cyp3a KO mice, as shown by Triazolam Oxidation Relative to Cyp3a KO mice, there is increased TRI metabolism due to the high catalytic activity of CYP3A4 in hCYP3A4/3A7_Cyp3a KO mice.
  • CYP3A4 plays a significant role in TRI metabolism in the liver, however TRI can also be extensively metabolised in the mouse.
  • CYP3A4 is catalytically active in CYP3A4/3A7_Cyp3a KO mice, as shown by Triazolam Oxidation A. Triazolam oxidation results showing catalytic activity of CYP3A4 in the liver of CYP3A4/3A7 Cyp3a knockout mice B. Triazolam oxidation results showing catalytic activity of CYP3A4 in the duodenum of CYP3A4/3A7 Cy ⁇ 3a knockout mice.
  • CYP3A4 is catalytically active in CYP3A4/3A7 Cyp3a KO mice, as shown by DBF Oxidation A. DBF oxidation results showing catalytic activity of CYP3A4 in the liver of CYP3A4/3A7 Cyp3a knockout mice B. DBF oxidation results showing catalytic activity of CYP3A4 in the duodenum of CYP3A4/3A7 Cyp3a knockout mice.
  • CYP3A4 is catalytically active in CYP3A4/3A7_Cyp3a KO mice, as shown by BQ Oxidation A. BQ oxidation results showing catalytic activity of CYP3A4 in the liver of CYP3A4/3A7 Cyp3a knockout mice B. BQ oxidation results showing catalytic activity of CYP3A4 in the duodenum of CYP3A4/3A7 Cyp3a knockout mice.
  • FIG. 20 Clinical chemistry analysis of plasma from C57BL/6J, hCYP3A4/3A7_Cyp3a KO, hCYP3A4_Cyp3a KO and Cyp3a KO mice
  • A total bilirubin (BIL-T)
  • B direct bilirubin
  • BIL-D C
  • AST aspartate aminotransferase
  • ALT alanine aminotransferase
  • FIG. 21 Clinical chemistry analysis of plasma from C57BL/6J, hCYP3A4/3A7_Cyp3a KO, hCYP3A4_Cyp3a KO and Cyp3a KO mice
  • A alkaline phosphatase
  • B albumin
  • FIG. 22 CYP3A4 protein expression in (A) liver and (B) intestinal microsomes from C57BL/6J, hCYP3A4/3A7_Cyp3a KO, hCYP3A4_Cyp3a KO and Cyp3a KO mice (+) - treated with PCN (100 mg/kg/2 days/IP); (-) - control animals treated with vehicle (corn oil). Each lane is a sample from one animal. lO ⁇ g of liver or 20 ⁇ g of intestinal microsomal protein were loaded. Blots were incubated in a polyclonal rabbit anti-CYP3A4 (Gentest, cat # 458234).
  • HLM - pooled male human liver microsomes (lO ⁇ g) (Gentest, cat # 452172); 3al l - murine Cyp3al l recombinant protein (0.1 pmol) (Dr. Henderson, Uni. of Dundee, UK); 3A4 - human CYP3A4 baculosomes (0.1 pmol) (Invitrogen, cat # P2377).
  • FIG. 23 CYP3A/Cyp3a protein expression in (A) liver and (B) intestinal microsomes from C57BL/6J, hCYP3A4_Cyp3a KO, hCYP3A4_Cyp3a KO and Cyp3a KO mice (+) - treated with PCN (100 mg/kg/2 days/IP); (-) - control animals treated with vehicle (corn oil). Each lane is a sample from one animal. lO ⁇ g of liver or 20 ⁇ g of intestinal microsomal protein were loaded. Blots were incubated in a polyclonal rabbit anti - rat CYP3A2 (Dr. Henderson, Uni. of Dundee, UK).
  • Figure 24 7-BQ oxidation by liver (A) and intestinal (B) microsomes from C57BL/6J, hCYP3A4/3A7_Cyp3a KO, hCYP3A4_Cyp3a KO and Cyp3a KO mice
  • Figure 25 DBF oxidation by liver (A) and intestinal (B) microsomes from C57BL/6J, hCYP3A4/3A7_Cyp3a KO, hCYP3A4_Cyp3a KO and Cyp3a KO mice.
  • Figure 26 ⁇ -Hydroxylation of triazolam by liver (A) and intestinal (B) microsomes from C57BL/6J, hCYP3A4/3A7_Cyp3a KO, hCYP3A4_Cyp3a KO and Cyp3a KO mice
  • a activities of samples from vehicle treated mice should be read using left Y axis scale, whereas activities of microsomes from PCN treated animals should be read using right Y axis scale.
  • FIG. 27 Agarose gel electrophoresis of RT-PCR products The reactions used CYP3A4 (lines 1 - 5) and CYP3A7 (lines 7-9) specific primers and total liver RNA.
  • CYP3A4 lines 1 - 5
  • CYP3A7 lines 7-9
  • specific primers and total liver RNA (1) - C57BL/6J; (2-3) - hCYP3A4/3A7_Cyp3a KO; (4-5) - hCYP3A4_Cyp3a KO; (6) - molecular weight marker lkb ladder, (7) - C57BL/6J; (8-9) - hCYP3A4/3A7_Cyp3a
  • the invention provides a method of introducing a heterologous replacement gene sequence into a host cell to replace an endogenous host gene target sequence, the method comprising: a) incorporating a pair of identical site-specific recombinase target (RT) sites of type I into the same allele of a host chromosome in separate homologous recombination steps such that the endogenous host gene target sequence that is to be replaced is flanked on each side by said identical type I RT sites; wherein one of the identical type I RT sites is flanked by a type II RT site positioned proximal to the type I RT site, wherein the type II RT site is different to the type I RT site such that it is heterospecif ⁇ c, and as such cannot interact with the type I RT site and; b) effecting recombination between said pair of type I site-specific recombination sites such that the endogenous host gene target sequence is excised, and whereby a residual type I RT
  • a heterologous replacement gene sequence is inserted into the chromosome of the host cell at the point in the chromosome where the endogenous host gene target sequence naturally occurs.
  • the first stage of the method of the present invention is the incorporation of a pair of identical type I RT sites into the host cell chromosome.
  • Methods for incorporation of the RT sites into the chromosome will be known to those of skill in the art, and are preferably performed by exploiting the process of homologous recombination.
  • Homologous recombination relates to the genetic mechanism which can be exploited to allow the insertion of a nucleic acid sequence into the host cell chromosome. The mechanism is initiated by the alignment of double-stranded host cell and exogenous nucleic acid sequences.
  • a double strand break in the host cell sequence and 5' to 3' exonuclease activity facilitates strand invasion, resulting in pairing of the homologous host cell and exogenous sequences through short regions of homology.
  • Subsequent chain elongation of the host cell sequence utilises the exogenous sequence as a template and resolution produces the host cell genomic sequence with the exogenous sequence located within it, whilst the exogenous sequence remains intact.
  • Methods for performing homologous recombination are known in the art and exploit regions of homology between exogenously supplied DNA molecules and the target chromosome to introduce the RT sites.
  • suitable targeted delivery systems will be clear to those of skill in the art and include the use of injected or targeted naked DNA, targeted liposomes encapsulating and/or complexed with the DNA, targeted retroviral systems and targeted condensed DNA such as protamine and polylysine- condensed DNA, or electroporation.
  • nucleic acid expression vectors polycationic condensed DNA or ligand linked DNA (see Curiel (1992) Hum Gene Ther 3:147-154; Wu (1989) J Biol Chem 264:16985-16987), and use of a gene transfer particle gun, (described in US 5,149,655).
  • naked DNA may also be employed, as is described in detail in international patent application WO90/11092. This list is provided by way of illustration only, and is not intended to be limiting.
  • a host cell is a stem cell, such as an iPS cell or an embryonic stem cell.
  • Embryonic stem (ES) cells are cultured cell lines of totipotent cells, wherein the cells, when introduced into an early embryo, will develop to populate all tissues of the developing organism. ES cells are preferred host cells according to the invention.
  • each of the type I RT sites is preferably incorporated into the host cell chromosome through a separate homologous recombination step, as described above.
  • Each of the separate homologous recombination reactions begins with the host cell chromosome and exogenous DNA which comprises the type I RT site, and regions of homology to the host cell chromosome region where homologous recombination is to occur.
  • the regions of homology are between 1 and 6kb, more preferably the regions of homology are between 1 and 4kb, most preferably, one of the regions of homology is 1 kb in length, and the other is either 3kb or 4kb in length.
  • the two type I RT sites are incorporated into the host cell chromosome so that the endogenous host gene target sequence which is to be replaced by the heterologous replacement gene sequence is flanked on each side by a type I RT site
  • the two type 1 RT sites are inserted into the endogenous host gene target sequences so that they are located less than 5mb from the host gene target sequence, more preferably the two type 1 RT sites are inserted into the endogenous host gene target sequence so that they are located less than 3mb from the host gene target sequence, and most preferably the two type 1 RT sites are inserted into the endogenous host gene target sequence so that they are located less than 2mb from the host gene target sequence.
  • the two type I RT sites are positioned in the same orientation as each other, to allow recombination between them in due course.
  • one of the type I RT sites incorporated into the host cell chromosome is flanked by a type II RT site, such that the type I RT site is positioned between the endogenous host gene target sequence and the type II RT site.
  • the type II RT site is preferably incorporated into the host cell chromosome through the same recombination step as its proximal type I RT site.
  • the exogenous DNA sequence utilised in the homologous recombination step should preferably contain the DNA sequence for the type I RT site and the type II RT site so that these can be introduced together.
  • the type I RT site and the type II RT site are positioned proximal to one another.
  • proximal is meant that the RT sites are positioned next to one another, close in proximity on the chromosome.
  • a "proximal" position resides within 100 nucleotides, preferably within 50 nucleotides, more preferably, within 40, 30, 20, 15, 10, 5 or less of another.
  • the type I RT site is different from the type II RT site, such that it is heterospecific, and as such cannot interact with the type I RT site.
  • the next stage of the method of the present invention is the excision of the endogenous host gene target sequence.
  • Excision is effected by effecting recombination between the two type I RT sites which flank the endogenous host gene target sequence.
  • the genome In order to effect recombination between the RT sites, the genome must be exposed to site-specific recombinase (SSR) activity, in the form of an SSR enzyme which recognises the type I RT sites. Exposure to SSR enzyme activity results in a DNA rearrangement determined by the disposition of the RT sites, which in a linear DNA molecule results in the intervening sequence being excised, or cut out.
  • SSR site-specific recombinase
  • SSR refers to any protein component of any recombinant system that mediates DNA rearrangements in a specific DNA locus, including SSRs of the integrase or resolvase/invertase classes (Abremski, K.E. and Hoess, R.H. (1992) Protein Engineering 5, 87-91; Khan, et al., (1991) Nucleic acids Res.
  • a residual type I RT site remains within the host cell chromosome, at the position previously occupied by the endogenous host gene target sequence, and the endogenous host gene target sequence is excised.
  • the endogenous host gene target sequence now exists within the cell as a free linear DNA molecule, which will be rapidly degraded by cellular exonucleases.
  • the next step in the method of the present invention is the provision of the heterologous replacement gene sequence, potentially as a linear nucleic acid molecule, but preferably contained within a vector of some kind such as a bacterial artificial chromosome (BAC), yeast artificial chromosome (YAC) or the like. Examples of suitable vectors are widely known in the art.
  • the heterologous replacement gene sequence is flanked on one side by a type I RT site, and on the other side by a type II RT site, whereby the type I RT site is the same type as the type I RT site inserted into the host cell chromosome, and the type II RT site is the same type as the type II RT site inserted into the host cell chromosome.
  • the type I RT site is different from the type II RT site, such that it is heterospecific, and as such cannot interact with the type I RT site.
  • the type I RT site flanking the heterologous replacement gene sequence is positioned in the same orientation as the type I RT site on the host cell chromosome, and the type II RT site at the other flank of the heterologous sequence is positioned in the same orientation as the type II RT site on the host cell chromosome, to allow effective recombination between the pairs of corresponding RT sites in due course.
  • recombination between the corresponding RT sites in the nucleic acid containing the heterologous replacement gene sequence and in the host cell chromosome is effected. These recombination steps preferably occur concurrently, and facilitate the introduction of the heterologous replacement gene sequence into the host cell chromosome at the position previously occupied by the endogenous host gene target sequence.
  • the proximal positioning of the type I and type II RT sites on the host cell chromosome leads to an increased efficiency of insertion of the heterologous replacement gene sequence compared to methods previously described in the prior art.
  • each of the type I RT sites incorporated into the host chromosome should preferably be linked to, and preferably contiguous to one or more selectable markers. These selectable markers function to allow monitoring of host cells, such as embryonic stem cells, into which the exogenous DNA has successfully integrated.
  • each type I RT site may be contiguous with one or more selectable markers.
  • each type I RT site is contiguous with 2 selectable markers.
  • each type I RT site is contiguous with at least one positive selection cassette, wherein a positive selection cassette will allow the detection of cells which have successfully incorporated the nucleic acid sequence.
  • the positive selection cassette allows selection by ensuring that only cells containing the nucleic acid sequence can survive in the growth medium.
  • each type I RT site is contiguous with at least one negative selection cassette, wherein a negative selection cassette will allow the detection of cells which have successfully had the nucleic acid sequence excised.
  • the negative selection cassette allows selection by ensuring that only cells not containing the nucleic acid sequence can survive in the growth medium.
  • each type I RT site is contiguous with one positive selection cassette and one negative selection cassette.
  • the one or more selectable markers are positioned so that the selectable markers lie between the endogenous host gene target sequence and the type I RT site, such that they are excised with the host gene sequence in due course.
  • the positive selection cassette is preferably a gene encoding some kind of resistance to a chemical compound to which the growing host cells can be exposed, such as an antibiotic.
  • examples include use of selectable markers conferring resistance to antibiotics added to the growth medium of cells, for instance the neomycin resistance marker conferring resistance to G418, hygromycin or puromycin. Further examples involve detection using nucleic acid sequences that are of complementary sequence and which will hybridise with, the nucleic acid sequence in accordance with the previous aspects of the invention. Examples would include Southern blot analysis, northern blot analysis and PCR.
  • the negative selection cassette is preferably a gene conferring sensitivity to a chemical compound. For example, a thymidine kinase (TK) gene may be used, and will confer sensitivity to ganciclovir.
  • TK thymidine kinase
  • the selectable markers are selected from a Thymidine kinase expression cassette, a hygromycin resistance gene and a promoter-less and ATG-deficient Neomycin cassette (5' ⁇ Neo) (see Seibler et ah, 2005, Nucl Acids Res. 33(7) e67).
  • one of the type I RT sites is contiguous to a Thymidine kinase expression cassette and 5' ⁇ Neo, and the other type I RT site is contiguous to a thymidine kinase expression cassette and a hygromycin resistance gene.
  • the 5' ⁇ Neo sequence that is located so as to be linked to one of the type I RT sites within the host cell chromosome, facilitates selection of cells due to the presence of a promoter and ATG within the host chromosome.
  • the basis of this concept is to use a promoterless and ATG-deficient neomycin cassette as a marker for integration. If this integrates randomly into the genome, this cassette is inactive and does not confer G418 resistance. It can be activated only by a precise insertion into an already prepared locus which contains the promoter and the ATG. This thus provides a stringent selection process for successful integration at a correct location in the chromosome.
  • the ATG is separated from the neomycin by a loxP site.
  • the complemented expressed neomycin sequence thus forms a fusion protein of amino acids encoded by the loxP site and the 3' half of the neomycin cassette.
  • the heterologous replacement gene sequence is on a vector, and that vector preferably contains one or more selectable markers.
  • the vector contains 2 selectable markers, preferably selected from a neomycin expression cassette and a hygromycin resistance gene.
  • the one or more selectable markers contained on the vector are preferably positioned between the type I RT site and the heterologous replacement gene sequence, and/or between the type II RT site and the heterologous replacement gene sequence.
  • at least one selectable marker is positioned on either side of the heterologous replacement gene sequence. More preferably one selectable marker is positioned on each side of the heterologous replacement gene sequence.
  • This selection system has the advantage that it is entirely directed by the selection marker genes introduced into the constructs by the experimenter. Therefore, the method of the present invention can be utilised in any embryonic stem cell, without the requirement for an initial selection pressure. This is in contrast to the method of Wallace et al, which can only be performed in an HPRT-def ⁇ cient (hprf) embryonic stem cell line.
  • the host chromosome is modified so as to contain one or more further RT sites in addition to the pair of type I RT sites and the type II RT site.
  • the host chromosome contains two additional RT sites as illustrated in Figure 1. More preferably the host chromosome contains one type III RT site and one type IV RT site. These additional RT sites are incorporated into the host cell chromosome by homologous recombination in the same manner as described previously for the type I and type II RT sites.
  • the additional RT sites are incorporated concurrently with the type I and type II RT sites.
  • the type II RT site incorporated into the host chromosome is flanked by a type III RT site, such that the type II RT site is positioned between the type I RT site and the type III RT site.
  • the type I RT site present in the host chromosome which is not flanked proximally by a type II RT site is flanked by a type IV RT site, such that the type I RT site is positioned between the endogenous host gene target sequence and the type IV RT site.
  • the vector contains one or more further RT sites in addition to the type I RT site and the type II RT site.
  • the vector contains two additional RT sites. More preferably the vector contains one type III RT site and one type IV RT site.
  • the additional RT sites are positioned within the vector so that they are flanked by the type I or type II RT site.
  • the type III RT site within the vector is located such that the type III RT site is positioned between the type II RT site and the heterologous replacement gene sequence. More preferably, the type III RT site is positioned between the heterologous replacement gene sequence and the one or more selectable markers, such that the one or more selectable markers are positioned between the type II RT site and the type III RT site.
  • the type IV RT site within the vector is located such that the type IV RT site is positioned between the type I RT site and the heterologous replacement gene sequence. More preferably, the type IV RT site is positioned between the heterologous replacement gene sequence and the one or more selectable markers, such that the one or more selectable markers are positioned between the type I RT site and the type IV RT site.
  • the additional RT sites present on the vector are aligned in the same direction as the corresponding RT sites in the host cell chromosome, so as to allow their recombination together in due course. Insertion of the heterologous replacement gene sequence into the host cell chromosome through SSR mediated recombination at the corresponding type I and type II RT sites positioned on the vector and the host cell chromosome, as described above, results in concurrent insertion of the additional RT sites into the host cell chromosome
  • Two separate recombination steps may then be effected between corresponding additional type III and type IV RT sites incorporated into the host chromosome.
  • the two additional recombination steps result in the excision of portions of DNA from the host cell chromosome, which included the selection cassettes.
  • the two additional recombination steps thus facilitate the deletion of all non-exogenous DNA, with the exception of the heterologous replacement gene sequence, and the two residual RT sites.
  • the two residual RT sites are a residual type III RT site and a residual type VI RT site.
  • SSR site specific recombinase
  • Exposure to SSR enzyme activity results in a DNA rearrangement determined by the disposition of the RT sites, which in a linear DNA molecule results in the intervening sequence being excised, or cut out.
  • SSR refers to any protein component of any recombinant system that mediates DNA rearrangements in a specific DNA locus, including SSRs of the integrase or resolvase/invertase classes (Abremski, K.E. and Hoess, R.H.
  • Such introduction can occur by the introduction of the SSR protein directly into the cell, or by the introduction of an exogenous gene encoding the SSR, which is subsequently expressed.
  • suitable targeted delivery systems for delivery of a gene encoding the SSR will be clear to those of skill in the art and include the systems described above.
  • In vivo recombination may be desirable if a transgenic organism has been produced, as described below. Site-specific recombination may then be effected by inducing activity of the SSR within the transgenic organism. Successful exploitation of site-specific recombination to alter genotype in living systems generally requires strategies to regulate the recombination event. This can be done by controlling expression of the recombinase mRNA, or protein (Baubonis and Sauer (1993) Nucl Acids Res. 21, 2025- 2029; Sauer B, (1994) Curr Opin Biotechnol 5:521-7; Rajewsky et al, (1996) J Clin Invest 98, 600-3; Metzger and Feil, (1999) Curr. Opinions Biotechnology 10, 470-476), such that the expression pattern achieved is confined to the times and places at which these tissue specific elements are active. Expression can be controlled in a tissue-specific pattern e.g. albumin-Cre in the liver.
  • Induction may thus be effected by inducing transcription of the SSR, inducing translation of the SSR, or removing an inhibitor from the SSR.
  • an SSR may be artificially introduced into the transgenic organism.
  • site-specific recombination can be effected within the transgenic organism, so resulting in the excision of the endogenous host gene target sequence and the concomitant production of a transgenic organism containing the heterologous replacement gene sequence in place of the endogenous host gene target sequence.
  • site-specific recombination can be effected in vivo by crossing a transgenic mouse with a deleter strain mouse.
  • the term "deleter strain” as used herein relates to a mouse expressing the site-specific recombinase in its germline, which can be crossed with a transgenic mouse to effect excision of the mouse target gene sequence. In this manner, in vivo recombination produces offspring heterozygous for the gene of interest.
  • transgenic mouse will therefore result in the production of progeny, with cells containing the mouse chromosome altered to contain the human replacement gene sequence and the site-specific recombinase, resulting in the excision of the mouse target gene and the functional humanisation of the cells.
  • Such a transgenic mouse will therefore be heterozygous for humanisation of the specific gene or cluster of genes.
  • the site-specific recombinase only to be expressed in a certain tissue of the recombinase strain mouse. It is known in the art that deletion of certain genes or clusters of genes may be lethal or may have sublethal phenotypic effects. Furthermore, replacing such genes with their human equivalents may not prevent lethality. In these circumstances, it may be possible to overcome any such problems of lethality by expressing the site-specific recombinase only in certain tissues, for example, the liver. This will be particularly advantageous if a specific gene is known to be essential in a certain tissue, as expression of the site-specific recombinase in this manner allows the mouse gene to persist in those tissues.
  • the SSR may be albumin-Cre.
  • Albumin-Cre is a specific variant of the SSR Cre which acts on the RT site LoxP.
  • Albumin-Cre is expressed only in the liver, and will therefore allow the mouse target sequence to persist in all tissues except the liver, overcoming possible problems of lethality, whilst providing a functionally humanised liver.
  • two heterozygous mice produced according to the methodology above may be crossed to produce a transgenic mouse that is homozygous for the human allele of the gene or genes of interest. Crossing two heterozygous transgenic mice will produce a proportion of progeny that are homozygous for the humanised allele.
  • transgenic non-human animal is produced de novo so as to include all of the aforementioned features, by the methods as hereinafter disclosed.
  • site-specific recombination event be effected in a somatic cell which could then be used as a nuclear transfer donor cell in order to make a colony of cloned mice according to the methodology of WO00/51424 or a variation thereof.
  • a transgenic animal according to the present invention is produced by crossing.
  • a mouse which still includes unwanted sequences between RT sites could be crossed with mouse expressing an SSR enzyme.
  • transgenic mouse is produced de novo so as to include all of the aforementioned features, by the methods as hereinafter disclosed.
  • none of the type I RT site, the type II RT site, the type III RT site, and the type IV RT site are the same, such that each type of RT site is heterospecific with respect to each of the other types of RT sites, and as such that none of the RT sites can interact with another RT site of a different type.
  • Preferred recombinase proteins are selected from the group consisting of: FLP recombinase, Cre recombinase, Dre recombinase, R recombinase from Zygosaccharomyces rouxii plasmid pSRl, a recombinase from the Kluyveromyces drosophilarium plasmid pKDl, a recombinase from the Kluyveromyces waltii plasmid pKWl, Trpl from the Bacillus transposon Tn4430, any component of the ⁇ Int recombination system, phiC31, any component of the Gin recombination system, or variants thereof.
  • the list is provided by way of example only, and is not intended to be limiting.
  • the site-specific recombination sites are chosen from loxP, Iox5171, Iox511, F3 and FRT.
  • the type I RT sites is loxP.
  • the type II RT site is Iox5171.
  • the type III RT site is FRT.
  • the type IV RT site is F3.
  • these RT sites can be interchanged such that Ioxl517 is type I, loxP is type II and so on.
  • any other heterospecific mutant of any of the RT sites could be used.
  • any heterospecific mutant of loxP, e.g. Iox511, could be used.
  • the heterogenous replacement gene sequence is introduced into the host cell on a vector.
  • the vector may preferably be a normal cloning vector, a Bacterial Artificial Chromosome or a Yeast Artificial Chromosome.
  • the vector is a BAC.
  • the optional vector contains the heterologous replacement gene sequence, which may comprise one or more gene(s) or segments of genes.
  • the heterologous replacement gene sequence may also comprise the regulatory regions associated with the one or more gene(s) of segments of genes.
  • the vector also comprises a type I RT site and a type II RT site, which flank the heterologous replacement gene sequence, and one or more selectable markers.
  • the endogenous host gene target sequence is the endogenous host gene target sequence
  • the host cell of the present invention may be any prokaryotic or eukaryotic cell in which it is possible for homologous recombination to take place, including bacteria, yeast, animal and plant cells.
  • the host cell is preferably a eukaryotic cell, more preferably a stem cell, such as an ES cell or an iPS cell (see Takahashi et al., Nat Protoc. 2007;2(12):3081-9; Yamanaka, Cell Prolif. 2008 Feb;41 Suppl 1 :51-6).
  • the host embryonic stem cell is a mammalian stem cell, such as a mammalian ES cell.
  • the mammalian embryonic stem cell is a mouse embryonic stem cell.
  • the invention may be implemented using any one of a number of genes, as will be clear to those of skill in the art. There is no technical limitation to the type of genes that may be exchanged between host cell target and heterologous replacement.
  • the invention is illustrated herein using a P450 gene cluster, in which the mouse Cyp3A, Cyp2C, or
  • Cyp2D cluster is replaced by the human equivalent cluster.
  • P450 genes are interesting candidates for humanisation, particularly on a null background, since such systems allow the human metabolic response to drug molecules to be assessed in the absence of interference from competing murine systems.
  • the genes are often very large, although they are generally clustered together in families of similar function. Accordingly, the methods of the invention lend themselves particularly well to the study of these humanised systems.
  • the expression product of the host cell target gene retains the same, similar, equivalent or identical function as the heterologous replacement gene.
  • the genes may be functionally equivalent, and/or structurally homologous.
  • the host cell target gene and heterologous replacement gene may share a degree of homology.
  • such homology will be greater than 30%, greater than 40%, greater than 50%, greater than 60%, greater than 70%, greater than 80%, greater than 90%, or even greater than 95%.
  • the endogenous host gene target sequence excised from the host cell chromosome will be defined by the position of the type I RT sites, which recombine to excise the DNA segment contained between them.
  • the position of the type I RT sites is dependant upon the location of the regions of homology between the host cell chromosome and the exogenous DNA segments containing the type I RT sites. Therefore, it will be apparent to one skilled in the art that any number of genes or gene segments can be excised from the host cell chromosome using the method of the present invention.
  • the regulatory regions associated with the endogenous host gene target sequence can be excised, or can remain in the host cell chromosome, depending upon the position of the type I RT sites.
  • the regulatory regions associated with the endogenous host gene target sequence may become operatively linked to the heterologous replacement gene sequence.
  • the advantage of this approach is that the endogenous gene expression pattern will be seen, and gene expression will be controlled in the same manner as it is in the unmodified host cell. This may have important implications for genes which are not normally expressed in the host cell.
  • the heterologous replacement gene sequence may preferably comprise cDNA, genomic DNA, or a mixture of the two.
  • Genomic DNA is advantageous in many circumstances because the fidelity of splicing will be retained. However, it may only be necessary to retain those introns where the majority of splice events take place, such that the remainder of the sequence can be cDNA. This can simplify the cloning process, particularly where the genomic DNA comprises large introns; in such cases the larger introns may not be included provided that splice isoforms are not coded for in this area of the genomic DNA.
  • heterologous replacement gene sequence is defined by the position of the type I and type II RT sites present in the vector, with the entire nucleic acid sequence between these two RT sites being inserted into the host cell chromosome, upon recombination with the corresponding RT sites present in the host cell chromosome.
  • the heterologous replacement gene sequence can therefore correspond to a gene segment, a whole gene, or a number of genes.
  • the heterologous replacement gene sequence may include regulatory sequences associated with the gene(s), or gene segment. These regulatory sequences would therefore be inserted into the host cell chromosome as part of the heterologous replacement gene sequence.
  • the regulatory sequences may be the regulatory sequences normally associated with the heterologous gene(s) or gene segment, and the gene(s) or gene segment would remain under the control of the regulatory sequences which normally control the gene(s) or gene segment. This may be advantageous as it would allow the heterologous replacement gene sequence to be expressed in the host cell in the same manner as it would normally be expressed. However, as described above, it may also cause expression problems.
  • the regulatory sequences associated with the gene(s) or gene segment may be heterologous sequences normally not associated with the gene(s) or gene segment included within the heterologous replacement gene sequence.
  • the regulatory sequences may be tissue specific regulatory sequences, including but not limited to regulatory sequences including the albumin promoter, the apoE promoter or the villin promoter.
  • the heterologous replacement gene sequence is a mammalian gene sequence.
  • the mammalian replacement gene sequence is a human replacement gene sequence. Provision of knockout lines
  • cell lines may be generated that contain a knockout of a particular endogenous gene or gene cluster.
  • the endogenous gene or cluster of genes is a member of the Cytochrome P450 family. Examples include the Cyp3a, Cyp2c and Cyp2d clusters.
  • the knockout cell line is stable.
  • stable is meant that the knockout cell line is able to be maintained in a viable form in cell culture for a minimum of 1 week. In other embodiments the knockout cell line is able to be maintained in a viable form for a minimum of 2 weeks, 3 weeks, 4 weeks, 1 month, 6 months, 1 year, 2 years or more.
  • a stable cell line is one which can be passaged at least 5 times, at least 10 times, at least 20 times, at least 30 times, at least 50 times, at least 100 times, at least 200 times or more whilst remaining viable.
  • the cell line used to produce the knockout cell line is a mammalian cell line.
  • the mammalian cell line is a mouse cell line.
  • the mouse cell line is a mouse stem cell line.
  • the mouse stem cell line is a mouse ES cell line.
  • the production of a stable knockout cell line is advantageous because such a pre- prepared knockout cell line can be used for the insertion of a heterologous replacement gene sequence according to the method described above.
  • the pre-prepared knockout cell line allows fewer steps to be performed in ES cells at the time of insertion of the heterologous replacement gene sequence, and will therefore increase the efficiency of transformation, and the frequency of correctly targeted clones.
  • the knockout cell lines described above may be used as the host cell line for the insertion of a heterologous replacement gene sequence or gene cluster according to the method described above.
  • the heterologous replacement gene sequence is a mammalian heterologous replacement gene sequence or gene cluster.
  • the mammalian heterologous replacement gene sequence is a human heterologous replacement gene sequence or gene cluster.
  • the human heterologous replacement gene sequence encodes a member of the Cytochrome P450 family.
  • the member of the Cytochrome P450 family may be a CYP3 A, a CYP2C or a CYP2D gene or gene cluster. Examples of CYP3A, CYP2C and CYP2D genes are CYP3A4, CYP3A5, CYP2C9, CYP2C19 or CYP2D6.
  • the knockout cell line used as the host cell line for the insertion of a heterologous replacement gene sequence contains a knockout of the gene or gene cluster which corresponds to the gene or gene cluster contained within the heterologous replacement gene sequence.
  • the heterologous replacement gene sequence used for insertion into a knockout cell line may be the same heterologous replacement gene sequence described above.
  • the heterologous replacement gene sequence may contain regulatory elements associated with the gene or gene cluster.
  • such regulatory elements are endogenous to the gene or gene cluster contained within the heterologous replacement gene sequence.
  • the regulatory elements may be tissue-specific regulatory elements. Examples of tissue-specific regulatory elements are the albumin, apoE and villin promoters.
  • transgenic organism produced by a method of any one of the embodiments of the invention described above.
  • Such an organism contains a heterologous replacement gene sequence at the position previously occupied by the endogenous host gene target sequence, and the corresponding endogenous host gene target sequence has been deleted.
  • the transgenic organism is a transgenic mammal
  • the deleted endogenous host gene target sequence is a mammalian gene target sequence
  • the transgenic mammal is a transgenic mouse
  • the deleted endogenous host gene target sequence is a mouse gene target sequence
  • the heterologous replacement gene sequence is a mammalian heterologous replacement gene sequence, and within a further aspect of the invention, the heterologous replacement gene sequence is a human replacement gene sequence.
  • altered stem cells such as ES cells of the invention containing the heterologous replacement gene sequence, may be inserted into a blastocyst. Conventionally, blastocysts are isolated from a female mammal, of corresponding species to the embryonic stem cell, about 3 days after it has mated. It is to be understood that up to 20 altered embryonic stem cells may be simultaneously inserted into such a blastocyst, preferably about 16.
  • the embryonic stem cell will become incorporated into the developing early embryo, preferably by its transplantation into a pseudo-pregnant mammal which has been induced so as to mirror the characteristics of a pregnant mammal.
  • the blastocyst containing the altered embryonic stem cell, will implant into the uterine wall of the pseudo-pregnant mammal and will continue to develop within the mammal until gestation is complete.
  • the altered embryonic stem cell will proliferate and divide so as to populate all tissues of the developing transgenic mammal, including its germ-line.
  • the created transgenic mammal may be a chimera, containing altered and non-altered cells within each somatic tissue and within the germ- line.
  • the pseudo-pregnant mammal is a pseudo-pregnant mouse
  • the altered cell is a mouse embryonic stem cell, as depicted in Figure 4.
  • the chimeric transgenic mammal generated by the method described above may be crossed with another chimeric transgenic mammal generated by the method described above, and the resulting progeny tested to identify a mammal homozygous for the inserted heterologous gene replacement sequence.
  • Methods which may be used to identify a mammal homozygous for the inserted heterozygous replacement gene sequence will be apparent to a person skilled in the art.
  • homozygotes may be identified by taking the tail tip of the mammal, PCR amplifying the section of the genome of interest, and sequencing the gene cluster of interest.
  • a probe specific for the heterologous gene replacement sequence may be used to identify homozygotes.
  • a single or multiple humanised mammal line produced according to any of the methods described above, wherein the host cell is a mammalian knockout cell line, as described above.
  • the host cell is a mammalian knockout cell line, as described above.
  • Such an organism contains a heterologous replacement gene sequence at the position previously occupied by the endogenous host gene target sequence, before the knockout cell line was produced.
  • the humanised mammal is a mouse.
  • humanised stem cells such as ES cells generated from knockout cell lines produced according to the invention and containing the heterologous replacement gene sequence, may be inserted into a blastocyst.
  • blastocysts are isolated from a female mammal, about 3 days after it has mated. It is to be understood that up to 20 altered embryonic stem cells may be simultaneously inserted into such a blastocyst, preferably about 16.
  • the embryonic stem cell will become incorporated into the developing early embryo, preferably by its transplantation into a pseudo-pregnant mammal which has been induced so as to mirror the characteristics of a pregnant mammal.
  • the blastocyst containing the altered embryonic stem cell
  • the altered embryonic stem cell will proliferate and divide so as to populate all tissues of the developing transgenic mammal, including its germ-line.
  • the created transgenic mammal may be a chimera, containing altered and non-altered cells within each somatic tissue and within the germ- line.
  • the chimeric transgenic mammal may be humanised for a gene or gene cluster belonging to the Cytochrome P450 family.
  • the Cytochrome P450 family may be a CYP3A, CYP2C or CYP2D gene or gene cluster.
  • the CYP3A, CYP2C or CYP2D gene may be CYP3A4, CYP3A5, CYP2C9, CYP2C19 or CYP2D6.
  • the chimeric transgenic mammal may contain the human CYP3A4, CYP3A5, CYP2C9, CYP2C19 or CYP2D6 gene cluster under the control of a tissue specific promoter.
  • the tissue specific promoter may be the albumin, apoE or villin promoter. As described in more detail above, this may be advantageous for genes or gene clusters, deletion of which may be lethal, or have sub-lethal phenotypic effects in certain tissues.
  • the chimeric transgenic mammal generated by the method described above may be crossed with another chimeric transgenic mammal generated by the method described above, and the resulting progeny tested to identify a mammal homozygous for the inserted heterologous gene replacement sequence.
  • Methods which may be used to identify a mammal homozygous for the inserted heterozygous replacement gene sequence will be apparent to a person skilled in the art.
  • homozygotes may be identified by taking a tissue sample, such as a tail tip from the mammal, PCR amplifying the section of the genome of interest, and sequencing the gene cluster of interest.
  • a probe specific for the heterologous gene replacement sequence may be used to identify homozygotes.
  • chimeric or homozygous humanised mammals which are humanised for different genes or gene clusters may be crossed in order to generate multiple humanised mammal lines.
  • one or more of a Cyp3a knockout humanised for CYP3A4, a Cyp3a knockout humanised for CYP3A5, a Cyp2c knockout humanised for CYP2C9 a Cyp2c knockout humanised for CYP2C19, or a Cyp2d knockout humanised for CYP2D6 may be crossed.
  • two, three, four or five of the humanised mammals may be crossed.
  • one or more of the human gene clusters may be under the control of a tissue specific promoter.
  • two, three, four or five of the human gene clusters may by under the control of a tissue specific promoter.
  • one or more of the human gene clusters may be under the control of the albumin, apoE or villin promoters.
  • two, three, four or five of the human gene clusters may be under the control of the albumin, apoE or villin promoters.
  • crossing one or more of the chimeric or humanised mammals which are humanised for different genes or gene clusters may result in the production of a double, triple, quadruple, or quintuple humanised mammal line.
  • further crossing and testing may be required to produce a mammal line homozygous for the double, triple, quadruple or quintuple humanisation.
  • a quadruple humanised mammal line is produced, wherein the mammal line has the endogenous Cyp3a and Cyp2c gene clusters knocked out, and the human CYP3A4, CYP3A5, CYP2C9 and CYP2C19 genes inserted.
  • one or more of the recited human genes are under the control of a tissue specific promoter.
  • two, three or four of the human genes may by under the control of a tissue specific promoter.
  • one or more of the human genes may be under the control of the albumin, apoE or villin promoters.
  • two, three or four of the human genes may be under the control of the albumin, apoE or villin promoters.
  • This approach to mammal humanisation is advantageous because it allows the production of a quadruple humanised mammal line using pre-prepared knockout mammal ES cells, and therefore requires substantially less effort than previous methods used for the production of a quadruple humanised mammal line.
  • the number of steps required to produce a quadruple humanised mammal line using this method is equivalent to the number of steps required to generate a double humanised mammal line using conventional methods. This reduction in the number of steps will increase the efficiency of humanised mammal line production.
  • this approach can be used to generate a multiple humanised mammal line which is humanised for a gene(s) or gene cluster different from genes of the Cytocliromoe P450 gene family.
  • genes include PXR and CXR.
  • a first basic targeting vector (Cyp3a57) containing a Hygromycin, Thymidine Kinase (TK) and ZsGreen expression cassette, and a loxP, Iox5171 and frt site was constructed in pBluescript (pBS).
  • pBS pBluescript
  • the translational start ATG and the corresponding promoter is separated from the 5' ⁇ Neo cassette in frame by the loxP site, such that additional amino acids encoded by the loxP site are fused to the N-terminus of Neomycin giving rise to a functional protein resulting in G418 resistance upon expression.
  • the second targeting vector (Cyp3a59) was linearised with Not I and electroporated into the correctly targeted Cyp3a57 ES clones B-G12 described above.
  • 1 correctly targeted clone (A-B5) was identified, expanded and further analysed by Southern blot analyses as described above. This clone was confirmed as correctly targeted at both homology arms and without additional random integrations (data not shown).
  • BAC Bacterial Artificial Chromosome
  • ES cells were carried out as described in example 1.
  • Neomycin cassette in the human BAC is promoterless and truncated at the 5' end, G418 resistance can only be obtained by a base pair precise integration via the loxP site.
  • 3 were expanded and further analysed by PCR and Southern blot analyses. All three clones were confirmed as correctly targeted at both ends of the human BAC, as shown in Figure 7B, one of the 3 clones had an additional integration, as shown in Figure 8B.
  • Example 3 Analysis ofhCYP3A4/3A7_Cyp3a KO mice
  • the following example is included to allow comparison between a Cypa3a knockout mouse line and a hCYP3A4/3A7 Cyp3a knockout mouse line produced according to the method of the invention.
  • Data relating to a hCYP3A4 Cyp3a knock out mouse line are produced according to the "two-step cluster deletion and humanisation" strategy, and are included for comparison only. This method does not form part of the present invention.
  • the BAC clone RP11-757A13 (ImaGenes GmbH, Robert-R ⁇ ssle-Str.10, 13125 Berlin, Germany, ImaGenes Clone ID: RPCIB753A13757Q) was modified by red/ET recombineering, such that the existing lox sites in the BAC are replaced with appropriately located loxP and Iox5171 sites and a hygromycin and 5' deficient neomycin selection cassette were introduced.
  • heterospecific flipase recombinase (FIp) recognition sites frt and f3 were introduced into the BAC enabling the subsequent removal of the hygromycin and neomycin selection cassettes in vivo by Flp-mediated recombination and a polyA motif was used to terminate any potential transcription initiated from the endogenous mouse Cyp3a57 promoter, which has not been deleted.
  • FIp flipase recombinase
  • Cyp3a-deleted subclones derived from the parental clone A-B5 were used to insert the modified BAC carrying human CYP3A4 and CYP3A7 by Cre-mediated recombination.
  • 1x10 7 cells were electroporated under standard conditions with approximately 30 ⁇ g of supercoiled BAC DNA and 12 ⁇ g of the Cre-expression plasmid pCAGGScrepA as previously described (40) and selected with G418. Seven G418 resistant ES cell clones were obtained after the electroporation procedure. Three of the clones were expanded and further analysed by PCR and Southern blot with different suitable restriction enzymes, 5' and 3' external probes, and an internal neomycin probe.
  • CYP3A4 Low basal CYP3A4 mRNA was identified, however this did not translate into protein. PCN-induced CYP3A4 protein expression was identified in this line which was comparable to humans. CYP3A4 is catalytically active in the hCYP3A4_Cyp3a KO mice relative to Cyp3a KO mice. These observations indicate that the CYP3A4 protein expressed in the hCYP3A4_Cyp3a KO mouse line is functional. CYP3A4 protein/mRNA but not CYP3A7 was identified suggesting a new utility of this model in the developmental regulation of CYP3As.
  • CYP3A4 is highly catalytically active in the hCYP3A4/3A7_Cyp3a KO mice relative to Cyp3a KO mice.
  • Cyp3a proteins in the mouse result in much higher levels of murine- specific metabolites compared to humans which has unfavourable toxicological implications.
  • mice (obtaibed from Harlan (UK)
  • AU animals used were males.
  • the mice were housed on sawdust in solid-bottom polypropylene cages. No environmental enhancing materials were used during treatment.
  • the environment was controlled to provide conditions required by the Home Office for accommodation and husbandry of rodents.
  • the temperature was maintained within a range of 19-23 0 C and relative humidity within a range of 40-70%.
  • mice were uniquely numbered, by ear-punch or tail marking, and allocated to groups, as shown in Table 2.
  • An experiment card was placed on each cage and showed the project licence code, treatment given, study number, sex and individual numbers of the mice within.
  • Table 2 Transgenic mouse allocation
  • mice Prior to the start of the study, all mice were observed to ensure that they were physically normal and that they exhibit normal activity. Only mice exhibiting normal behaviour were accepted for the study. Any clinical abnormalities observed in individual animals were recorded in the study diary. A general assessment of condition was recorded in the study diary.
  • mice received either corn oil (vehicle) or PCN 100 mg/kg, daily, for 2 days by intraperitoneal (IP) injection according to the experimental design described in Table 3.
  • Dosing solutions were prepared at CXR Biosciences on the day of dosing by adding the vehicle (corn oil) to the requisite quantity of the PCN.
  • the concentration of PCN was the concentration of supplied chemical, without any correction for purity.
  • Excess dosing solution was stored at approximately 2-8°C for possible future analysis.
  • the volume of dosing solution was 10 mL/kg bodyweight. Approximately 24 h after the second dose, the mice were euthanized using a rising concentration of CO 2 . Blood was collected at termination by cardiac puncture into lithium/heparin coacted tubes for plasma preparation.
  • the body weight of each mouse was recorded at the start of the study and immediately prior to termination. Bodyweights were recorded electronically or manually and records of these weights were stored in the study file.
  • liver In order to weigh the liver, the gall bladder was removed, and then the liver was removed and weighed. Two samples of liver (approximately 5mm 3 ) were immediately flash frozen in a cryovial in liquid nitrogen then stored at approximately -70 0 C for RNA analysis. The remaining liver was weighed and immediately used for subcellular fractionation to homogenates and microsomes.
  • the liver/body weight ratio of the C57BL/6J mice significantly (P ⁇ 0.001) increased as a result of PCN administration as shown in Table 4.
  • the liver/body weight ratios of the control and treated transgenic mice could not be statistically compared as there was only one transgenic animal in each control group. All treated transgenic mice showed a decreased liver/body weight ratio compared to the treated wild type, although only in the Cyp3aKO group was this decrease statistically significant (P ⁇ 0.05).
  • Table 4 Body and liver weights
  • the liver/body weight ratios were compared with an unpaired t test (two tailed P values).
  • Plasma samples were produced by removing red blood cells by centrifugation (2,000 - 3,000 rpm for 10 min at 8-10 0 C). The supernatant (plasma) was stored on ice prior to clinical chemistry analysis. The pellet was discarded. Plasma samples from all animals were analysed for triglycerides, alanine aminotransferase, alkaline phosphatase, aspartate aminotransferase, albumin, cholesterol, bilirubin (total and direct), high and low density lipoproteins using the COBAS Integra 400+ (Roche), and the results are shown in Figures 19-21.
  • Plasma samples from PCN treated hCYP3A4_Cy ⁇ 3a KO mice demonstrated statistically significant increases in the level of cholesterol, low and high density lipoproteins, alanine transferase and alkaline phosphatase compared to the samples from treated C57BL/6J mice. The biological significance of this increase will have to be investigated using larger group sizes.
  • the values of plasma clinical chemistry parameters for all other samples fell within the known normal range for untreated C57BL/6J mice.
  • Table 5 shows the range of plasma clinical chemistry parameters of the untreated C57BL/6J mice.
  • mice 1 and mice 4 There was insufficient plasma from mouse 1 (control C57BL/6J) and mouse 4 (control hCYP3A4_Cyp3a KO) to perform cholesterol analysis.
  • Table 5 Normal range of selected plasma clinical chemistry in untreated wild type C57BL/6J mice
  • Values represent Mean ⁇ SEM for the following plasma analytes; ALP, ALT, AST, albumin, BIL-D, BIL-T, cholesterol, HDL, LDL and triglycerides. Maximum and minimum vales are also included. Data was generated by collating plasma clinical chemistry values across multiple studies generated using the COBAS 400+ Integra (Roche). There was insufficient plasma from mouse 1 (control C57BL/6J) and 5 mouse 4 (control hCYP3A4_Cyp3a KO) to perform cholesterol analysis.
  • the duodenum (first 10cm from the base of the stomach) was removed and flushed with ice cold PBS containing a protease inhibitor cocktail (Roche).
  • the first 2cm was but and placed into a 2ml cry vial containing ImI of TRIZOL (Sigma), flash frozen immediately, and then stored at approximately -70°C for Taqman ® analysis.
  • the remainder of the duodenum was placed in a ImI ciyovial and flash frozen immediately, and then stored at approximatley-70 o .
  • Liver microsomes were produced by preparing subcellular fractions from fresh livers. The livers were processed as described above to homogenates and microsomes. Aliquots from liver samples were stored at approximately -70° prior to analysis.
  • Frozen small intestines were homogenised in SET with protease cocktail inhibitor (Roche) and PMSF (mM) using a Polytron homogeniser. The homogenates were subjected to subcellular fractionation as described above. The microsomal fractions were stored at approximately -70° prior to analysis. Liver microsomes from C57BL/6J, hCYP3A4/3A7_Cyp3a KO, hCYP3A4_Cyp3a KO and Cyp3a KO mice were analysed by Western blotting using an antibody specific to CYP3A4 and the results are shown in Figure 22.
  • DBF (2 ⁇ M) was incubated with 5 ⁇ L liver or 25 ⁇ L intestinal microsomes in 50 mM HEPES buffer pH 7.4 (15 mM MgC12, 0.1 mM EDTA) at 37°C for approximately 50 sec before the reaction was started by addition of 20 ⁇ L NADPH (42 mg/mJL).
  • the total reaction volume was 1 mL.
  • Fluorescein fluorescence was recorded using an F-4500 fluorescence spectrophotometer (Hitachi), excitation 485 nm and emission 538 nm.
  • Fluorescein standard (10 ⁇ L, 25 ⁇ M) was injected into the reaction cuvette approximately 150 sec after the addition of NADPH. Slopes of the time course of the product accumulation were calculated using FL- Solution 2.0 (Hitachi).
  • Triazolam 50 ⁇ M was incubated with microsomes (2.5 ⁇ L liver microsomes or 6 ⁇ L intestinal microsomes) and NADPH (1.3 mM) in 50 mM HEPES buffer pH 7.4 (15 mM MgC12, 0.1 mM EDTA) at 37oC. The total reaction volume was 200 ⁇ L. After 15 min, the reaction was stopped by taking an aliquot (80 ⁇ L) of the reaction mixture and adding it to an equal volume of ice-cold acetonitrile.
  • 3A4_F__B get gaa agg aag act cag agg Tm: 59.8
  • RNA was prepared from liver tissue of humanised (hCYP3A4/3A7_Cyp3a KO (mouse 4) and hCYP3A4_Cyp3a KO (mouse 5)) and wild type C57BL/6J (mouse 1) mice using an RNeasy kit (QIAGEN, Cat No. 74104) according to the manufacturer's instructions, and purified using RNeasy kit (QIAGEN).
  • RT-PCR was conducted using a Superscript III One-Step RT-PCR Platinum Taq HiFi Kit (Invitrogen Corp. Cat. No. 12574-030) according to the manufacturer's protocol. The products of RT-PCR were separated by electrophoresis on an agarose gel. A DNA fragment of the predicted size was extracted from agarose gel, and then cloned into vector pCR4-TOPO using a TOPO TA Cloning kit for Sequencing (Invitrogen Corp. Cat. no. K4575-01).
  • PCR amplification 40 cycles of: 94°C 30 sec 54oC 30 sec 68°C 2 min Final extension: 68°C 5 min
  • mice 4 and 5 were extracted from the agarose gel and separately cloned into the pCR4/TOPO vector.
  • RNA sample isolated from humanised mouse 4 was analysed by RT-PCR using primers 3A7_F and 3 A7_R. No DNA product was observed in either wild type (mouse 1) or humanised (mouse 4) mice as shown in Figure 27.
  • CYP3A4 and CYP3A7 mRNA levels were performed by Q-PCR analysis using CYP3A4 and CYP3A7 specific primers. ⁇ -Actin was used as a reference gene.
  • the Q-PCR analysis of the liver and intestinal samples is summarised in Table 8.
  • Table 8 Average threshold cycle (Ct) and delta Ct fdCfl values for CYP3A4 f3A4).
  • CYP3A4 mRNA was confidently detected both in the liver and in small intestine of the control and treated humanised mice. CYP3A7 mRNA level was below the detection limit in the liver of the control hCYP3A4/3A7_Cyp3a KO mice. This data was consistent with the results from RT-PCR and sequencing of CYP3A4 and CYP3A7.
  • CYP3 A4 protein constitutive expression of CYP3 A4 protein was detected in liver microsomes of male hCYP3A4/3A7 mice using a CYP3A4 specific antibody. However the expression level of this enzyme was markedly lower than that of murine Cyp3a according to the results of the immunoblot for CYP3A/Cyp3a protein. Intestinal microsomes of C57BL/6J and hCYP3A4/3A7_Cyp3a KO mouse lines demonstrated similar expression of CYP3A/Cyp3a protein.
  • hepatic CYP3A4 in hCYP3A4_Cyp3a KO mice was below the detection limit of Western blotting and the intestinal sample from this strain demonstrated a very low intensity band of CYP3A4.
  • the immunoblot data were generally consistent with the activities in oxidation of the CYP3A4 specific substrates, although any statistical comparison was not possible as only one animal from each transgenic strain was available. Treatment with PCN resulted in strong induction of hepatic and intestinal CYP3A4 in both humanised lines.
  • CYP3A7 mRNA was undetectable in samples from the control animals.
  • CYP3A7 is the major CYP3A isoform expressed in human foetal liver, and undergoes a developmental switch in the first week of postnatal life, with CYP3A7 virtually disappearing concomitant with transcriptional activation of the CYP3A4 gene (Stevens et al., 2003; Hines, 2008).
  • a similar developmental switch has also been observed in the mouse (Cyp3al6 to Cyp3al l) (Stevens et al., 2003).
  • the mice used in this experiment were 9- 15 weeks old and therefore, the expression of CYP3A7 might be switched to the expression of CYP3A4.
  • Cyp2c cluster targeting vectors were produced as described in Example 1 for Cyp3a cluster targeting vectors.
  • Cre-mediated deletion of the Cyp2c cluster in double targeted ES cells was performed as described in Example 1 for Cre-mediated Cyp3a cluster deletion.

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Abstract

La présente invention concerne, en général, un procédé pour introduire une séquence de gène de remplacement hétérologue dans une cellule souche embryonnaire hôte pour remplacer une séquence cible de gène d’hôte endogène. En particulier, l’invention concerne un procédé pour insérer de grands segments d’ADN dans des cellules souches embryonnaires avec une efficacité améliorée, dans un premier temps en délétant la séquence cible de gène d’hôte endogène, et ensuite en utilisant deux sites cibles de recombinase (RT) à site spécifique positionnés à proximité l’un de l’autre pour insérer une séquence de gène de remplacement hétérologue dans le chromosome hôte.
EP09723802A 2008-03-26 2009-03-25 Insertion efficace d adn dans des cellules souches embryonnaires Withdrawn EP2271207A2 (fr)

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